preparing a single-cell suspension of immune cells from murine brain tissue

Preparing a Single-Cell Suspension of Immune Cells from Murine Brain Tissue

Pour the brain or spinal cord tissue with the media into a 100-millimeter Petri dish, and use forceps to move the tissue to the bottom. Mince the brain tissue with a sterile razor blade, and gather the tissue at the bottom of the plate. Add 3 milliliters of RPMI supplemented with 10% FCS to the Petri dish, then use a 10-milliliter serological pipette to resuspend the tissue in the media and transfer it to a 15-milliliter conical tube.
Add collagenase type I and DNase I to the tissue and incubate the tubes in a 37 degrees Celsius water bath for 40 minutes. Invert the tubes every 15 minutes to thoroughly mix the tissue with the enzymes. After incubation, add EDTA to each tube for a final concentration of 0.01 molar, and incubate the tubes for an additional five minutes to inactivate the collagenase.
Add 9 milliliters of RPMI, supplemented with 10% FCS to each tube, then, centrifuge the tubes at 450 g for 5 minutes at 4 degrees Celsius. Use a Pasteur pipette with a vacuum to aspirate the supernatant, taking care not to touch the cell pellet.
Add 3 milliliters of 100% stock isotonic density gradient solution to the cell pellet. Then, add additional RPMI 10% FCS media to bring the final volume to 10 milliliters and resuspend the cell pellet. Invert and mix the tube well. Then, insert a serological pipette with 1 milliliter of 70% stock isotonic density gradient solution into the bottom of the tube.
Slowly underlay the solution, being careful not to make bubbles. Remove the serological pipette from the tube, making sure not to disturb the gradient. Centrifuge the tube at 800 g for 30 minutes at 4 degrees Celsius, then aspirate the supernatant, including the myelin debris layer until 2 to 3 milliliters remain in the tube.
Use a 1-milliliter pipette to harvest the cell layer between the 30% and 70% density gradient and transfer it to a new 15-milliliter tube. Add RPMI 10% FCS media to bring the final volume to 15 milliliters, then centrifuge the cells at 450 g for 5 minutes at 4 degrees Celsius.

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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee. 
1. Preparing single-cell suspensions of brain and spinal cord tissue
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	<li>Transfer the brain or spinal cord tissue with media to the top of the 100 mm Petri dish by pouring the tissue and media from the tube. Using forceps, move the tissue to the bottom of the Petri dish. Finely mince the brain or spinal cord with a sterile razor blade. Using the ...

Source: DiSano, K. D., et al. <a href="https://app.jove.com/v/61166">Isolating Central Nervous System Tissues and Associated Meninges for the Downstream Analysis of Immune Cells.</a> J. Vis. Exp. (2020).
The video demonstrates the preparation of a single-cell suspension of immune cells from a murine brain tissue. It involves enzymatic digestion to release cells from the brain tissue, followed by density gradient centrifugation to isolate the immune cells based on their densities to obtain the single-cell suspension.

<img alt="Figure 1" src="/files/ftp_upload/22589/22589_Figure 1.jpg" /> 
Figure 1: Identification of CD45hi infiltrating immune cells in CNS tissues. (A) Gating strategy for the identification of CD45hi infiltrating immune cells (P1), CD45lo microglia (P2), and CD45- oligodendrocytes, astrocytes, and neurons among total live cells in spinal cords from sham-treated (red) or TMEV-IDD (blue) mice. Minimal CD45hi cells were detected in sham-treated brains and spinal cord...

All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee. 
1. Preparing single-cell ...

Begin with a murine brain with neural, non-neural, and immune cells within the brain&#39;s extracellular matrix or ECM.
Mince the tissue and resuspend it in a culture medium.
Transfer these tissue fragments to a tube and treat them with collagenase and DNase-I enzymes.
Collagenase digests the ECM, releasing individual cells, while DNase-I degrades free DNA to prevent cell clumping.
Then, add EDTA to inactivate the collagenase enzymes.
Add a culture medium. Centrifuge and remove the supernatant.
Add a density gradient solution and the culture medium to the cell pellet, creating a low-density gradient layer.
Mix and then underlay the solution with a high-density gradient solution to establish a density difference.
Centrifuge at low speed to separate immune cells at the interface, with lighter cell debris at the top and heavier neuronal and glial cells at the bottom.
Remove the upper layer, and collect the immune cells, and transfer them to another tube.
Centrifuge and remove the supernatant, then resuspend the cells in a medium, forming a single-cell suspension for downstream applications.

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Preparing a Single-Cell Suspension of Immune Cells from Murine Brain Tissue

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